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nmrlearner 03-28-2019 01:56 AM

Selective high-resolution DNP-enhanced NMR of biomolecular binding sites #DNPNMR
 
From The DNP-NMR Blog:

Selective high-resolution DNP-enhanced NMR of biomolecular binding sites #DNPNMR

Marin-Montesinos, Ildefonso, David Goyard, Emilie Gillon, Olivier Renaudet, Anne Imberty, Sabine Hediger, and Gaël De Paëpe. “Selective High-Resolution DNP-Enhanced NMR of Biomolecular Binding Sites.” Chemical Science 10, no. 11 (2019): 3366–74.


https://doi.org/10.1039/C8SC05696J.


Locating binding sites in biomolecular assemblies and solving their structures are of the utmost importance to unravel functional aspects of the system and provide experimental data that can be used for structurebased drug design. This often still remains a challenge, both in terms of selectivity and sensitivity for X-ray crystallography, cryo-electron microscopy and NMR. In this work, we introduce a novel method called Selective Dynamic Nuclear Polarization (Sel-DNP) that allows selective highlighting and identification of residues present in the binding site. This powerful site-directed approach relies on the use of localized paramagnetic relaxation enhancement induced by a ligand-functionalized paramagnetic construct combined with difference spectroscopy to recover high-resolution and high-sensitivity information from binding sites. The identification of residues involved in the binding is performed using spectral fingerprints obtained from a set of high-resolution multidimensional spectra with varying selectivities. The methodology is demonstrated on the galactophilic lectin LecA, for which we report well-resolved DNP-enhanced spectra with linewidths between 0.5 and 1 ppm, which enable the de novo assignment of the binding interface residues, without using previous knowledge of the binding site location. Since this approach produces clean and resolved difference spectra containing a limited number of residues, resonance assignment can be performed without any limitation with respect to the size of the biomolecular system and only requires the production of one protein sample (e.g. 13C,15N-labeled protein).


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